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人外周血白细胞的质膜流动性梯度

Plasma membrane fluidity gradients of human peripheral blood leukocytes.

作者信息

Collins J M, Scott R B, Grogan W M

机构信息

Department of Biochemistry, Medical College of Virginia Commonwealth University, Richmond 23298-0614.

出版信息

J Cell Physiol. 1990 Jul;144(1):42-51. doi: 10.1002/jcp.1041440107.

Abstract

The shape of the fluidity gradient of the outer hemileaflet of the plasma membrane of normal, living, human white blood cells was determined using a series of n-(9-anthroyloxy) fatty acid probes where n = 2, 3, 6, 7, 9, 11, 12, and 16, to establish a baseline for future studies on the consequences of various pathological states. Fluorescence uptake and steady-state anisotropy values were obtained with a flow cytometer capable of continuous recording over time of vertical and horizontal emission intensities, with the output of these intensities as calculated anisotropy values. The fluorescence uptake of all of the membrane probes was rapid up to about 15 min. The magnitudes of the uptake of fluorescence was, for the n-(9-anthroyloxy) series, in the order 2 greater than 3 greater than 6 greater than 7 greater than 9 greater than 11 = 12 = 16 for neutrophils, lymphocytes, and monocytes. Anisotropy values were constant from 5 to 30 min after addition of the various probes. The orders of the anisotropy magnitudes, indicative of the shapes of the fluidity gradient, were, for neutrophils, 6 greater than 7 greater than 9 greater than 2 = 3 = 11 = 12 greater than 16, for lymphocytes, 7 greater than 6 greater than 9 greater than 11 greater than 2 = 3 greater than 11 = 12 greater than 16, and for monocytes, 9 greater than 7 greater than 6 greater than 11 greater than 2 = 3 greater than 12 greater than 16. The kinetics of anisotropy from 1 to 5 min after addition of the probes differed for each of the three cell types. Probes with an n-value less than or equal to the maxima (n = 6, neutrophils; n = 7, lymphocytes; n = 9, monocytes) rapidly (1.2 min) reached equilibrium, whereas those probes with n-values greater than the maxima took progressively longer times to equilibrate as n increased. This behavior is consistent with the existence of an energy barrier just below the approximate region sensed by the probes, which would correspond to just below 6AS for neutrophils, 7AS for lymphocytes, and 9AS for monocytes.

摘要

使用一系列n -(9 - 蒽氧基)脂肪酸探针(其中n = 2、3、6、7、9、11、12和16)来确定正常、活的人类白细胞质膜外半层流动性梯度的形状,从而为未来关于各种病理状态后果的研究建立一个基线。通过一台能够随时间连续记录垂直和水平发射强度,并将这些强度输出计算为各向异性值的流式细胞仪,获得荧光摄取和稳态各向异性值。所有膜探针的荧光摄取在大约15分钟内都很快。对于中性粒细胞、淋巴细胞和单核细胞,n -(9 - 蒽氧基)系列荧光摄取量的大小顺序为2大于3大于6大于7大于9大于11 = 12 = 16。在添加各种探针后5到30分钟内,各向异性值保持恒定。对于中性粒细胞,指示流动性梯度形状的各向异性大小顺序为6大于7大于9大于2 = 3 = 11 = 12大于16;对于淋巴细胞,顺序为7大于6大于9大于11大于2 = 3大于11 = 12大于16;对于单核细胞,顺序为9大于7大于6大于11大于2 = 3大于12大于16。添加探针后1到5分钟内,三种细胞类型各自的各向异性动力学有所不同。n值小于或等于最大值(中性粒细胞中n = 6;淋巴细胞中n = 7;单核细胞中n = 9)的探针迅速(1.2分钟)达到平衡,而n值大于最大值的那些探针随着n值增加达到平衡所需时间逐渐变长。这种行为与在探针所感知的近似区域正下方存在一个能量屏障相一致,这对应于中性粒细胞约6AS下方、淋巴细胞约7AS下方和单核细胞约9AS下方。

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